Kinetic Characterization of dUTPase from Escherichia coli

Larsson, Gunilla; Nyman, Per Olof; Kvassman, Jan

doi:10.1074/jbc.271.39.24010

Cited by 94 publications

(171 citation statements)

References 25 publications

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“…The reaction is initiated by the attack of the nucleophilic water, leading to an associative pathway for the phosphate cleavage that has been identified in solution and in several enzymes that carry out phosphate cleavage or transfer (see e.g., Florián et al [53][54] and Klahn et al 55 ). This mechanism is also consistent with the experimentally observed pH change that is used to directly follow the reaction kinetics, 56 and with the lack of observed intermediates for the phosphate hydrolysis. 33 It is found in E. coli dUTPase that two protons transfer to the reaction medium in a concerted mode, immediately following the rate limiting step.…”

supporting

confidence: 86%

Mutations Decouple Proton Transfer from Phosphate Cleavage in the dUTPase Catalytic Reaction

et al. 2015

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Most enzymes present a catalytic mechanism where one or more proton transfer events occur coupled tightly together with the enzymatic chemical reaction. We show here that inactivating mutations decouple this proton transfer step from the phosphate cleavage reaction in dUTPase. Homotrimeric dUTPase enzymes catalyze the hydrolysis of dUTP to dUMP and pyrophosphate, using largely similar structural and functional groups as most AAA+ enzymes. dUTPases typically use a single Mg 2+ ion as a cofactor in the active site that is formed by direct protein-protein contacts including all three protomers. Here we focus on the C-terminal arm structural motif, which has sequence and functional similarities to P-loop motifs, and is required for catalysis. In this work, we have studied the functional roles of the C-terminal arm in ligand binding and catalysis by using QM/MM (quantum mechanics/molecular mechanics) calculations in conjunction with site-directed mutagenesis experiments. We also present a new method to assess the metal ion coordination symmetry during the catalytic reaction. Using this new implementation, we identified that the coordination symmetry follows a consistent pattern in the three systems studied, reaching the most symmetrical state near the transition states. We found that the phosphate cleavage proceeds with a concerted bimolecular (A N D N ) mechanism with a loose dissociative transition state, and that it is coupled with a proton transfer step involving a unanimously conserved Asp residue. We show that the main mechanistic effect of the lack of the C-terminal arm is to decouple the phosphate cleavage from the subsequent proton transfer step, resulting in a highbarrier altered reaction pathway.

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supporting

confidence: 86%

Mutations Decouple Proton Transfer from Phosphate Cleavage in the dUTPase Catalytic Reaction

et al. 2015

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“…This conformational change is realized by intricate subunit interactions as the C terminus of one subunit crosses over its neighboring subunit and adopts an ordered conformation to contact the substrate bound in the active site of the third subunit. In the bacterial enzyme, detailed functional investigations (2,30,33,34), in agreement with the crystal structure in complex with the nucleotide dUDP (28), indicate that the ␥ phosphate of the substrate is indispensable in inducing the closed conformer, and after catalytic cleavage the active site pops open. In the case of the human enzyme, the crystal structure suggests the retaining of the closed conformer even with the product dUMP (24), but there are no functional data published.…”

supporting

confidence: 57%

“…Experiments to identify the physiological isoforms of fly dUTPase are in progress in our laboratory. 2 Both the N and C termini of fly dUTPase may contain subcellular localization segments sensitive to proteolysis (Fig. 5), arguing for their exposed character and accessibility that might be helpful in binding to potential transport proteins.…”

Section: Discussionmentioning

confidence: 99%

“…This method was used to conveniently follow activity during purification and trypsinolysis, as well as to record substrate saturation curves with the dUTP analogues dCTP and dTTP. The enzyme kinetic parameters k cat and K M were determined either from substrate saturation curves or from the entire progress curve of dUTP cleavage using the integrated Michaelis-Menten equation, as described previously (2,33). Metal ion requirement was tested in separate experiments, using Chelex-treated components.…”

Section: Methodsmentioning

confidence: 99%

“…The enzyme dUTPase catalyzes the hydrolysis of dUTP into dUMP and anorganic pyrophosphate using a metal ion (Mg 2ϩ ) (1,2). Through this reaction, the enzyme keeps the cellular dUTP/dTTP ratio at a low level by depleting the dUTP pool and contributing in parallel to dTTP biosynthesis (3).…”

mentioning

confidence: 99%

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Altered Active Site Flexibility and a Structural Metal-binding Site in Eukaryotic dUTPase

Kovari

Barábas

Takács

et al. 2004

Journal of Biological Chemistry

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dUTPase is responsible for preventive DNA repair via exclusion of uracil. Developmental regulation of the Drosophila enzyme is suggested to be involved in thymine-less apoptosis. Here we show that in addition to conserved dUTPase sequence motifs, the gene of Drosophila enzyme codes for a unique Ala-Pro-rich segment. Kinetic and structural analyses of the recombinant protein and a truncation mutant show that the Ala-Pro segment is flexible and has no regulatory role in vitro. The homotrimer enzyme unfolds reversibly as a trimeric entity with a melting temperature of 54°C, 23°C lower than Escherichia coli dUTPase. In contrast to the bacterial enzyme, Mg 2؉ binding modulates conformation of fly dUTPase, as identified by spectroscopy and by increment in melting temperature. A single well folded, but inactive, homotrimeric core domain is generated through three distinct steps of limited trypsinolysis. In fly, but not in bacterial dUTPase, binding of the product dUMP induces protection against proteolysis at the tryptic site reflecting formation of the catalytically competent closed conformer. Crystallographic analysis argues for the presence of a stable monomer of Drosophila dUTPase in crystal phase. The significant differences between prototypes of eukaryotic and prokaryotic dUTPases with respect to conformational flexibility of the active site, substrate specificity, metal ion binding, and oligomerization in the crystal phase are consistent with alteration of the catalytic mechanism and hydropathy of subunit interfaces.

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Flexible glycine rich motif ofEscherichia coli deoxyuridine triphosphate nucleotidohydrolase is important for functional but not for structural integrity of the enzyme

Vértessy

1997

Proteins

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Deoxyuridine triphosphate nucleotidohydrolase (dUTPase), a ubiquitous enzyme of DNA metabolism, has been implicated as a novel target of anticancer and antiviral drug design. This task is most efficiently accomplished by X-ray crystallography of the relevant protein-inhibitor complexes. However, the topic of the present investigation, a glycine-rich strictly conserved structural motif of dUTPases, could not be located in the crystal structure of the Escherichia coli enzyme, probably due to its increased flexibility. The present work shows that removal of a C-terminal 11-residue fragment, including this motif, by limited trypsinolysis strongly impairs catalytic activity. Kinetic analysis of the intact and digested variants showed that kcat decreases 40-fold, while KM increases less than twofold upon digestion. The tryptic site was identified by mass spectrometry, amino acid analysis and N-terminal sequencing. The shortened enzyme variant retains the secondary, tertiary, and quaternary (trimeric) structure of the intact species as suggested by UV absorption, fluorescence and circular dichroism spectroscopy, and analytical gel filtration. Moreover, binding affinity of the shortened variant toward the substrate analogue MgdUDP is identical to the one displayed by the intact enzyme. I conclude that the glycine-rich motif is functionally relevant for E. coli dUTPase. It may play a role in enzymatic catalysis by contributing to the formation of the catalytically potent enzyme-substrate complex.

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Kinetic Characterization of dUTPase from Escherichia coli

Cited by 94 publications

References 25 publications

Mutations Decouple Proton Transfer from Phosphate Cleavage in the dUTPase Catalytic Reaction

Mutations Decouple Proton Transfer from Phosphate Cleavage in the dUTPase Catalytic Reaction

Altered Active Site Flexibility and a Structural Metal-binding Site in Eukaryotic dUTPase

Flexible glycine rich motif ofEscherichia coli deoxyuridine triphosphate nucleotidohydrolase is important for functional but not for structural integrity of the enzyme

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